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Target Region Selection Is a Critical Determinant of Community Fingerprints Generated by 16S Pyrosequencing

机译:目标区域的选择是由16S焦磷酸测序产生的社区指纹的关键决定因素。

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摘要

Pyrosequencing of 16S rRNA genes allows for in-depth characterization of complex microbial communities. Although it is known that primer selection can influence the profile of a community generated by sequencing, the extent and severity of this bias on deep-sequencing methodologies is not well elucidated. We tested the hypothesis that the hypervariable region targeted for sequencing and primer degeneracy play important roles in influencing the composition of 16S pyrotag communities. Subgingival plaque from deep sites of current smokers with chronic periodontitis was analyzed using Sanger sequencing and pyrosequencing using 4 primer pairs. Greater numbers of species were detected by pyrosequencing than by Sanger sequencing. Rare taxa constituted nearly 6% of each pyrotag community and less than 1% of the Sanger sequencing community. However, the different target regions selected for pyrosequencing did not demonstrate a significant difference in the number of rare and abundant taxa detected. The genera Prevotella, Fusobacterium, Streptococcus, Granulicatella, Bacteroides, Porphyromonas and Treponema were abundant when the V1–V3 region was targeted, while Streptococcus, Treponema, Prevotella, Eubacterium, Porphyromonas, Campylobacer and Enterococcus predominated in the community generated by V4–V6 primers, and the most numerous genera in the V7–V9 community were Veillonella, Streptococcus, Eubacterium, Enterococcus, Treponema, Catonella and Selenomonas. Targeting the V4–V6 region failed to detect the genus Fusobacterium, while the taxa Selenomonas, TM7 and Mycoplasma were not detected by the V7–V9 primer pairs. The communities generated by degenerate and non-degenerate primers did not demonstrate significant differences. Averaging the community fingerprints generated by V1–V3 and V7–V9 primers providesd results similar to Sanger sequencing, while allowing a significantly greater depth of coverage than is possible with Sanger sequencing. It is therefore important to use primers targeted to these two regions of the 16S rRNA gene in all deep-sequencing efforts to obtain representational characterization of complex microbial communities.
机译:16S rRNA基因的焦磷酸测序可对复杂的微生物群落进行深入表征。尽管已知引物选择会影响测序产生的群落特征,但对深度测序方法的偏倚程度和严重性尚不十分清楚。我们测试了以下假设:靶向测序和引物简并性的高变区在影响16S pyrotag社区的组成中起重要作用。使用Sanger测序和4引物对焦磷酸测序分析了当前吸烟者慢性牙周炎深处龈下斑块。通过焦磷酸测序比通过桑格测序检测到更多物种。稀有类群占每个pyrotag社区的近6%,而不到Sanger测序社区的1%。但是,选择用于焦磷酸测序的不同目标区域在稀有和丰富分类单元的数量上没有显示出显着差异。当以V1–V3区域为靶标时,Prevotella,融合杆菌,链球菌,颗粒葡萄球菌,拟杆菌,卟啉单胞菌和梅毒螺旋体是丰富的,而V4–6引物在社区中以链球菌,梅毒螺旋体,Prevotella,真细菌,卟啉单胞菌,弯曲杆菌和肠球菌为主。 ,而V7–V9社区中最多的属是Veillonella,链球菌,真细菌肠球菌 Treponema Catonella Selenomonas 。瞄准V4-V6区域无法检测到融合细菌属,而 Selenomonas TM7 支原体则是V7–V9引物对未检测到。由简并引物和非简并引物产生的群落没有显示出显着差异。对由V1-V3和V7-V9引物产生的群落指纹进行平均可得到与Sanger测序相似的结果,同时所覆盖的深度比Sanger测序要大得多。因此,在所有深度测序工作中使用针对16S rRNA基因这两个区域的引物很重要,以获得复杂微生物群落的表征。

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